Fig. 6. Regulation of mntH gene mRNA by manganese and iron in the parent strain and a fur mutant.

mRNAs were analyzed by quantitative real-time PCR from cells grown in media supplemented with no metal (black bars), 50 μM MnCl₂ (white bars), 20 μM FeCl₃ (striped bars) or both MnCl₂ and FeCl₃ (stippled bars). The data are expressed as the relative starting quantity (SQ) of the respective mRNAs normalized to the housekeeping gene gapA, and presented as the average of triplicate samples ± the standard deviation.